Figure 4.

The role of G-protein coupling in serelaxin-mediated cAMP accumulation in human primary umbilical vascular cells. Pretreatment of HUASMC (n = 6) in (A) and of HUVSMC (n = 6) in (B) with the selective Gα_s inhibitor NF449 (10 μM, 30 min) caused a rightward shift and reduced the E-max of the cAMP CRC to serelaxin without modifying the shape of the curve. Pretreatment of HUASMC (n = 7) in (C) and of HUVSMC (n = 6) in (D) with the selective Gα_i/o inhibitor NF023 (10 μM, 30 min) reduced the E-max of the cAMP CRC to serelaxin and changed the shape of the curve observed with HUVSMC (D) from bell-shaped to sigmoidal. In both (E) HUASMC (n = 6) and (F) HUVSMC (n = 6), pretreatment with both NF449 and NF023 completely abolished serelaxin-mediated cAMP responses, showing that the responses result entirely from RXFP1 receptors interaction with G proteins. In (G) HUASMC (n = 6) and in (H) HUVSMC (n = 6), pretreatment with filipin III (1 μg·mL⁻¹, 1 h), which disrupts lipid rafts, mimicked the effect of the Gα_i/o inhibitor NF023 – reducing E-max and converting CRCs from bell-shaped to sigmoidal in HUVSMC.